首页> 美国卫生研究院文献>Journal of Bacteriology >Bacteriophage Attachment Sites Serological Specificity and Chemical Composition of the Lipopolysaccharides of Semirough and Rough Mutants of Salmonella typhimurium
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Bacteriophage Attachment Sites Serological Specificity and Chemical Composition of the Lipopolysaccharides of Semirough and Rough Mutants of Salmonella typhimurium

机译:鼠伤寒沙门氏菌半粗糙突变体和粗糙突变体脂多糖的噬菌体附着位点血清学特异性和化学组成

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摘要

Extracted lipopolysaccharides (LPS) from one smooth, one semirough, and five rough mutants of Salmonella typhimurium LT2 or LT7, for which the chemical structure of the polysaccharide chain had been elucidated by using methylation analysis, were characterized with passive hemagglutination inhibition and phage inactivation experiments. Each addition of a sugar residue to a LPS from chemotype Rc was reflected in changed serological reactivity and phage-inhibiting activity of a collection of bacteriophages of the isolated LPS. Thus, certain criteria can be established for a classification of rough mutants of S. typhimurium. The observation that the serological RII specificity corresponds to a completed common core polysaccharide was verified. The serological RI specificity was found in LPS with terminal d-galactose I residues. One of the mutants, SL733, yielded a LPS which cross-reacted with anti-O5 factor serum although the polysaccharide was virtually free from contaminating O-specific material. The O5 reactivity was destroyed by alkaline treatment of SL733 LPS. The smooth- and rough-specific Felix O-l (FO) and the rough-specific 6SR and Br2 phages were shown to have their receptors in the LPS. There was a good correlation between the adsorption rate constant to whole cells and the phage inhibiting activity of isolated LPS suggesting that the LPS exert the major influence on the attachment of these phages to the bacteria. The polysaccharide structures in the LPS necessary for attachment of the 6SR and Br2 phages were defined. It was found that measuring the phage-inhibiting properties of isolated LPS as PhI50 (LPS concentration required to inactivate 50% of the phages under defined conditions) was a more sensitive method for a characterization of the LPS than the serological and chemical assays used.
机译:通过甲基化分析阐明了鼠伤寒沙门氏菌LT2或LT7的一个平滑,一个半粗糙和五个粗糙突变体中提取的脂多糖(LPS),并通过被动血凝抑制和噬菌体灭活实验对其进行了表征。 。从化学型Rc向LPS的糖残基的每次添加反映为分离的LPS的一组噬菌体的血清反应性和噬菌体抑制活性的改变。因此,可以为鼠伤寒沙门氏菌的粗突变体的分类建立某些标准。证实了血清学RII特异性对应于完成的普通核心多糖的观察。在具有末端d-半乳糖I残基的LPS中发现了血清学RI特异性。突变体之一SL733产生了一种与抗O5因子血清交叉反应的LPS,尽管该多糖实际上没有污染O特异材料。通过碱处理SL733 LPS破坏O5反应性。光滑特异性和粗糙特异性的Felix O-1(FO)以及粗糙特异性的6SR和Br2噬菌体在LPS中具有其受体。在全细胞上的吸附速率常数与分离的LPS的噬菌体抑制活性之间存在良好的相关性,这表明LPS对这些噬菌体对细菌的附着起主要作用。定义了6SR和Br2噬菌体附着所必需的LPS中的多糖结构。已发现,测量分离的LPS的噬菌体抑制特性为PhI50(在规定条件下灭活50%的噬菌体所需的LPS浓度)比使用的血清学和化学测定法更灵敏地表征LPS。

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